4 resultados para PFGE
em Chinese Academy of Sciences Institutional Repositories Grid Portal
Resumo:
Amphioxus is a crucial organism for the study of vertebrate evolution. Although a genomic BAC library of Branchiostoma floridae has been constructed, we report here another BAC library construction of its distant relative species Branchiostoma belcheri. The amphioxus BAC library established in present study consists of 45,312 clones arrayed in one hundred and eighteen 384-well plates. The average insert fragment size was 120 kb estimated by Pulsed Field Gel Electrophoresis (PFGE) analysis of 318 randomly selected clones. The representation of the library is about 12 equivalent to the genome, allowing a 99.9995% probability of recovering any specific sequence of interest. We further screened the library with 4 single copied Amphi-Pax genes and identified total of 26 positive clones with average of 6.5 clones for each gene. The result indicates this library is well suited for many applications and should also serve as a useful complemental resource for the scientific community.
Resumo:
Yeast strain Saccharornyces cerevisiae was irradiated with different doses of 85 MeV/u Ne-20(10+) to investigate DNA damage induced by heavy ion beam in eukaryotic microorganism. The survival rate, DNA double strand breaks (DSBs) and DNA polymorphic were tested after irradiation. The results showed that there were substantial differences in DNA between the control and irradiated samples. At the dose of 40 Cy, the yeast cell survival rate approached 50%, DNA double-strand breaks were barely detectable, and significant DNA polymorphism was observed. The alcohol dehydrogenase II gene was amplified and sequenced. It was observed that base changes in the mutant were mainly transversions of T-->G and T-->C. It can be concluded that heavy ion beam irradiation can lead to change in single gene and may be an effective way to induce mutation.
Resumo:
目的:重离子辐射生物学效应机理和哺乳动物细胞对重离子的辐射敏感性机理在目前仍颇有争议,是辐射生物学研究的热点。材料与方法:采用兰州重离子研究装置(HIRFL)加速的碳、氧、氩等重离子辐照体外培养的贴壁细胞,以集落法测定细胞的存活率;辐照琼脂糖包埋的细胞样品或DNA样品,以脉冲场凝胶电泳(PFGE)分析辐照诱导的DNA双链断裂(DSB)。结果:1.DNA片段释放百分比(PR)值随着剂量的增加而增加,在超过一定剂量后趋于一个准阈值;而DNA断裂水平与剂量之间呈线性关系,DSB产额为O.19-1.55DSBs/100Mbp/Gy;以~(60)Co γ射线为参照,得到重离子辐照诱导DSB的相对生物效率(RBE)为0.73-2.72。2.剂量率是影响DSB诱导及其片段分布的因素之一,剂量率越大,DSB产额越高,DSB诱导截面越大。但剂量率低可以使片段的非随机分布更为明显。3.重离子辐照诱导的DSB可以修复,修复方式主要是小片段连接成大的片段。4.无论是~(60)Coγ射线,还是碳、氧、氩等重离子,直接辐照DNA分子和辐照完整细胞诱导DSB的比值为1.64-2.64。说明细胞组分对DNA分子有一定的保护作用。5.辐照DNA分子诱导DSB的RBE随传能线密度(LET)的变化而变化,但IBE最大值远小于细胞失活的RBE最大值。结论:1.重离子辐照DNA分子诱导的DSB初始产额与细胞失活机理之间有一定的联系,但以此来解释细胞失活还不够充分;而不可修复的DSB才是细胞失活最主要的原因。2.细胞对重离子的辐射敏感性与DSB初始产额的关系不明显,但与细胞对DSB的修复能力高低密切相关。3.重离子辐照诱导的DSB片段是非随机分布的,其产生与DNA序列有关,即DNA分子上存在对重离子辐照敏感的位点。重离子辐照沉积的能量可以直接或间接地沿DNA链迁移,从而使得DNA分子上相对较弱或亲电性较强的化学键优先断裂。敏感位点即这些相对较弱或亲电性较强的化学键,而这 种化学键的产生是与敏感位点邻近的几个核苷酸相互作用的结果,即敏感位点应该是一段DNA序列。
Resumo:
TdT-mediated dUTP-biotin nick end labeling (TUNEL) is a sensitive and valid method for detecting DNA cleavage in programmed cell death (PCD). Using this method, DNA cleavage was observed in Laminaria japonica sporophytic tissues, which were infected with alginic acid decomposing bacterium. It was found that DNA cleavage occurred 5 min after the infection, the fragments with 3'-OH groups of cleaved nuclear DNA increased with time of infection and spread from the infection site. Although no typical DNA ladder (200 bp/ 180 bp) was detected by routine agarose gel electrophoresis, the cleavage of nuclear DNA fragments of 97 similar to 48.5 kb could be detected by pulsed field gel electrophoresis (PFGE). By using CaspGLOW(TM) fluorescein active caspase-3 staining method, caspase-3 activity has been detected in response to the infection of alginic acid decomposing bacterium. Our results are similar to the observations in hypersensitive response (HR) of higher plant, suggesting that the rapid cell death of L. japonica infected by alginic acid decomposing bacterium might be involved in PCD, and indicating that the occurrence of PCD is an active defense process against the pathogen's infection.
